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Efficient PRNP deletion in bovine genome using gene-editing technologies in bovine cells

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Title
Efficient PRNP deletion in bovine genome using gene-editing technologies in bovine cells
Author(s)
WooJae Choi; Eunji Kim; Soo-Young Yum; ChoongIl Lee; JiHyun Lee; JoonHo Moon; Sisitha Ramachandra; Buddika Oshadi Malaweera; JongKi Cho; Jin-Soo Kim; SeokJoong Kim; Goo Jang
Subject
Cattle embryos, ; Immortalization, ; Knockout, ; PRNP, ; TALEN
Publication Date
2015-07
Journal
PRION, v.9, no.4, pp.278 - 291
Publisher
LANDES BIOSCIENCE
Abstract
Even though prion (encoded by the PRNP gene) diseases like bovine spongiform encephalopathy (BSE) are fatal neurodegenerative diseases in cattle, their study via gene deletion has been limited due to the absence of cell lines or mutant models. In this study, we aim to develop an immortalized fibroblast cell line in which genome-engineering technology can be readily applied to create gene-modified clones for studies. To this end, this study is designed to 1) investigate the induction of primary fibroblasts to immortalization by introducing Bmi-1 and hTert genes; 2) investigate the disruption of the PRNP in those cells; and 3) evaluate the gene expression and embryonic development using knockout (KO) cell lines. Primary cells from a male neonate were immortalized with Bmi-1and hTert. Immortalized cells were cultured for more than 180 days without any changes in their doubling time and morphology. Furthermore, to knockout the PRNP gene, plasmids that encode transcription activator-like effector nuclease (TALEN) pairs were transfected into the cells, and transfected single cells were propagated. Mutated clonal cell lines were confirmed by T7 endonuclease I assay and sequencing. Four knockout cell lines were used for somatic cell nuclear transfer (SCNT), and the resulting embryos were developed to the blastocyst stage. The genes (CSNK2A1, FAM64A, MPG and PRND) were affected after PRNP disruption in immortalized cells. In conclusion, we established immortalized cattle fibroblasts using Bmi-1 and hTert genes, and used TALENs to knockout the PRNP gene in these immortalized cells. The efficient PRNP KO is expected to be a useful technology to develop our understanding of in vitro prion protein functions in cattle. © 2015 Taylor & Francis Group, LLC
URI
https://pr.ibs.re.kr/handle/8788114/2389
DOI
10.1080/19336896.2015.1071459
ISSN
1933-6896
Appears in Collections:
Center for Genome Engineering(유전체 교정 연구단) > 1. Journal Papers (저널논문)
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